固醇载体蛋白 2 基因缺失对培养的原代小鼠肝细胞中高密度脂蛋白介导的胆固醇流出的影响。
Effect of sterol carrier protein-2 gene ablation on HDL-mediated cholesterol efflux from cultured primary mouse hepatocytes.
机构信息
Departmens of Physiology and Pharmacology, Texas Veterinary Medical Center, Texas A & M University, College Station, TX 77843-4466, USA.
出版信息
Am J Physiol Gastrointest Liver Physiol. 2010 Jul;299(1):G244-54. doi: 10.1152/ajpgi.00446.2009. Epub 2010 Apr 15.
Although HDL-mediated cholesterol transport to the liver is well studied, cholesterol efflux from hepatocytes back to HDL is less well understood. Real-time imaging of efflux of 22-(N-(7-nitrobenz-2-oxa-1,3-diazol-4-yl)-amino)-23,24-bisnor-5-cholen-3beta-ol (NBD-cholesterol), which is poorly esterified, and [(3)H]cholesterol, which is extensively esterified, from cultured primary hepatocytes of wild-type and sterol carrier protein-2 (SCP-2) gene-ablated mice showed that 1) NBD-cholesterol efflux was affected by the type of lipoprotein acceptor, i.e., HDL3 over HDL2; 2) NBD-cholesterol efflux was rapid (detected in 1-2 min) and resolved into fast [half time (t((1/2))) = 2.4 min, 6% of total] and slow (t((1/2)) = 26.5 min, 94% of total) pools, consistent with protein- and vesicle-mediated cholesterol transfer, respectively; 3) SCP-2 gene ablation increased efflux of NBD-cholesterol, as well as [(3)H]cholesterol, albeit less so due to competition by esterification of [(3)H]cholesterol, but not NBD-cholesterol; and 4) SCP-2 gene ablation increased initial rate (2.3-fold) and size (9.7-fold) of rapid effluxing sterol, suggesting an increased contribution of molecular cholesterol transfer. In addition, colocalization, double-immunolabeling fluorescence resonance energy transfer, and electron microscopy, as well as cross-linking coimmunoprecipitation, indicated that SCP-2 directly interacted with the HDL receptor, scavenger receptor class B type 1 (SRB1), in hepatocytes. Other membrane proteins in cholesterol efflux [SRB1 and ATP-binding cassettes (ABC) A-1, ABCG-1, ABCG-5, and ABCG-8] and several soluble/vesicle-associated proteins facilitating intracellular cholesterol trafficking (StARDs, NPCs, ORPs) were not upregulated. However, loss of SCP-2 elicited twofold upregulation of liver fatty acid-binding protein (L-FABP), a protein with lower affinity for cholesterol but higher cytosolic concentration than SCP-2. Ablation of SCP-2 and L-FABP decreased HDL-mediated NBD-cholesterol efflux. These results indicate that SCP-2 expression plays a significant role in HDL-mediated cholesterol efflux by regulating the size of rapid vs. slow cholesterol efflux pools and/or eliciting concomitant upregulation of L-FABP in cultured primary hepatocytes.
尽管人们对 HDL 介导的胆固醇向肝脏的转运进行了深入研究,但对肝细胞内胆固醇向 HDL 的外排过程了解甚少。应用实时成像技术研究 22-(N-(7-硝基苯并-2-氧代-1,3-二唑-4-基)-氨基)-23,24-双降-5-胆甾烯-3β-醇(NBD-胆固醇)和[(3)H]胆固醇从野生型和甾醇载体蛋白-2(SCP-2)基因敲除小鼠原代培养肝细胞中的外排,结果表明:1)NBD-胆固醇的外排受脂蛋白受体的类型影响,即 HDL3 比 HDL2 高;2)NBD-胆固醇的外排迅速(在 1-2 分钟内检测到),并分为快速(半衰期(t((1/2))) = 2.4 分钟,占总外排的 6%)和慢速(t((1/2)) = 26.5 分钟,占总外排的 94%)池,分别与蛋白和囊泡介导的胆固醇转移一致;3)SCP-2 基因敲除增加了 NBD-胆固醇和[(3)H]胆固醇的外排,尽管由于[(3)H]胆固醇酯化的竞争,其作用较小,但 NBD-胆固醇除外;4)SCP-2 基因敲除增加了快速外排甾醇的初始速率(2.3 倍)和大小(9.7 倍),提示分子胆固醇转移的贡献增加。此外,共定位、双免疫荧光共振能量转移和电子显微镜以及交联免疫沉淀表明,SCP-2 可直接与肝细胞中的 HDL 受体清道夫受体 B 型 1(SRB1)相互作用。胆固醇外排的其他膜蛋白(SRB1 和 ABCA-1、ABCG-1、ABCG-5 和 ABCG-8)和几种促进细胞内胆固醇转运的可溶性/囊泡相关蛋白(StARDs、NPCs、ORPs)并未上调。然而,SCP-2 的缺失引起肝脂肪酸结合蛋白(L-FABP)的两倍上调,L-FABP 与胆固醇的亲和力较低,但细胞浆浓度高于 SCP-2。SCP-2 和 L-FABP 的缺失降低了 HDL 介导的 NBD-胆固醇外排。这些结果表明,SCP-2 的表达通过调节快速和慢速胆固醇外排池的大小以及/或在原代培养的肝细胞中同时上调 L-FABP,在 HDL 介导的胆固醇外排中发挥重要作用。
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